Immobilization of modified penicillin G acylase on Sepabeads carriers

An approach to stable covalent immobilization of chemically modified penicillin G acylase from Escherichia coli on Sepabeads® carriers with high retention of hydrolytic activity and thermal stability is presented. The two amino-activated polymethacrylate particulate polymers with different spacer lengths used in the study were Sepabeads® EC EA and Sepabeads® EC HA. The enzyme was first modified by cross-linking with polyaldehyde derivatives of starch in order to provide it with new useful functions. Such modified enzyme was then covalently immobilized on amino supports. The method seems to provide a possibility to couple the enzyme without risking a reaction at the active site which might cause the loss of activity. Performances of these immobilized biocatalysts were compared with those obtained by the conventional method with respect to activity and thermal stability. The thermal stability study shows that starch-PGA immobilized on Sepabeads EC-EA was almost 4.5-fold more stable than the conventionally immobilized one and 7-fold more stable than free non-modified PGA. Similarly, starch-PGA immobilized on Sepabeads EC-HA was around 1.5- fold more stable than the conventionally immobilized one and almost 9.5-fold more stable than free non-modified enzyme.     

Immobilization of heavy metals by Pseudomonas putida CZ1/goethite composites from solution

Bacterial–mineral composites are important in the retention of heavy metals due to their large sorption capacity under a wide range of environmental conditions. This study provides the first quantitative comparison of the metal-binding capacities of P. putida CZ1–goethite composite to its individual components. When the same amount (on a dry weight basis) of living and nonliving cells of P. putida CZ1, goethite or their composites was separately exposed to solutions of 0.5 mM Cu(II) and Zn(II) in 0.01 M KNO₃, the living cells removed the largest quantity of heavy metals. The results of calculated metal retention values indicated that the adsorption of goethite to bacteria has not mask or neutralize chemically reactive adsorption sites normally available to metal ions. Moreover, the nonliving cells–goethite composite retained approximately 82% more Zn than that predicted by their individual behavior. The preferential association of Zn with P. putida CZ1 was observed by TEM and EDS analyses of a mixture consisting of the bacteria and goethite. Desorption of Cu and Zn with 1.0 M CH₃COOK solution from P. putida CZ1 and goethite indicated the differences in the functional groups able to bind heavy metals.     

Immobilization of flower-like ZnO on activated carbon fibre as recycled photocatalysts

Research on Chemical Intermediates - ZnO was grown on the surface of activated carbon fibre (ACF) by a hydrothermal method to form a recyclable photocatalyst. With an increase in hydrothermal time...     

Immobilization of Aspergillus nidulans SU04 cellulase on modified activated carbon

The present study deals with the immobilization of Aspergillus nidulans SU04 cellulase onto modified activated carbon (MAC). The effect of contact time, cellulase concentration, MAC dosage, and temperature for maximum immobilization percentage and immobilization capacity is investigated. The equilibrium nature of immobilization is described by Langmuir and Freundlich isotherms. The kinetic data were tested using the pseudo first order. The activation energy of immobilization was evaluated to be 11.78?J?mol^?1. Results of the thermodynamic investigation indicate the spontaneity (?G <0), slightly endothermic (?H >0), and irreversible (?S >0) nature of the sorption process. Entropy and enthalpy were found to be 41.32 J?mol^?1?mg^?1 and 10.99?kJ?mol^?1, respectively. The Gibbs free energy was found to be ?22.79?kJ?mol^?1. At 80?rpm, 323?K, 2?h, 5?mg of MAC, immobilization capacity was 4.935?mg cellulase per mg of MAC from an initial cellulase concentration of 16?mg?ml^?1 with retention of 70% of native cellulase activity up to 10 cycles of batch hydrolysis experiments. The diffusion studies that were carried out revealed the reaction rate as ??mol?min^?1. At optimized conditions, immobilized cellulase had a higher Michaelis?CMenten constant, K _m of 1.52?mmol and a lower reaction rate, V _max of 42.2???mol?min^?1, compared with the free cellulase, the K _m and V _max values of which were 0.52?mmol and 18.9???mol?min^?1, respectively, indicating the affinity of cellulase for MAC matrix.     

Effects of different carriers on the production of isoflavone powder from soybean cake

The objectives of this study were to use soybean cake as the raw material for the production of isoflavone powder and compare the effects of different carriers as well as drying methods on the powder quality. Results showed that with spray drying, a level of 40% maltodextrin as carrier produced the highest yield (mass) of isoflavone powder, followed by 10% gelatin and 1% sodium alginate. However, a reversed trend was observed for the isoflavone content. With 1% sodium alginate, freeze drying generated the greatest yield of isoflavone powder, followed by vacuum drying and spray drying. The isoflavone content also exhibited the same tendency. With poly-gamma-glutamic acid (gamma-PGA) as carrier, all six levels studied (0.57, 0.28, 0.14, 0.028, 0.014 and 0.003%) were capable of forming powder containing high amounts of total isoflavone, which was comparable to that using 1% sodium alginate by freeze drying. Both high- and low-molecular-weight gamma-PGA showed similar effects in terms of powder yield and isoflavone content.     

Immobilization of proteins on gold coated porous membranes via an activated self-assembled monolayer of thioctic acid

A new methodology for efficient protein (e.g., antibodies, enzymes, etc.) immobilization on microporous nylon membranes for use in a variety of bioanalytical systems is introduced. The method utilizes an activated self-assembled monolayer (SAM) of thioctic acid on gold coated forms of the membranes. Via a carbodiimide mediated reaction, the protein is anchored to the gold surface through an amide bond with the terminal carboxyl group of the adsorbed thioctic acid. The immobilization efficiency is high (95% for a monoclonal immunoglobulin G(IgG) and the surface bound protein appears to be stable enough to resist any displacement by other proteins in a matrix as complex as serum. Immunological activity of immobilized antibody is retained as demonstrated via use of such membrances in colorimetric ELISA for human chorionic gonadatropin (hCG). The high protein immobilization efficiency, the high tensile strength of microporous nylon membranes, and the excellent electrochemical characteristics of gold make this approach very attractive for preparing biomembranes that should be useful in affinity chromatography, electrochemical immunosensing systems, flow-through enzyme reactors, etc.     

Immobilization and surface characterization of NeutrAvidin biotin-binding protein on different hydrogel interlayers

For a number of potential applications, it is desirable to immobilize avidin class molecules onto solid supports and exploit their ability to bind biotinylated molecules with high affinity. NeutrAvidin molecules were surface immobilized in various ways. In this study, NeutrAvidin was covalently attached by carbodiimide chemistry onto carboxyl groups of polyacrylic acid and carboxymethyl-dextran hydrogel interlayers. A third strategy involved the affinity "docking" of NeutrAvidin onto a biotinylated poly(ethylene glycol) interlayer. These three interlayers were selected for their low nonspecific binding of proteins, which was expected to minimize surface binding of NeutrAvidin by nonspecific interfacial adsorption. X-ray photoelectron spectroscopy (XPS) analyses allowed detailed characterization of the multilayer fabrication steps. An ELISA assay was used to measure NeutrAvidin activity, which varied with the surface immobilization route. Atomic force microcopy (AFM) force measurements showed that the hydrogel interlayer contributed to a repulsive force and verified the specific interaction between biotinylated AFM tips and the NeutrAvidin surfaces. When a solution of free biotin was injected into the AFM liquid cell, the force curve changed substantially and became identical to that recorded between surfaces carrying no NeutrAvidin, indicating that the free solution biotin had displaced NeutrAvidin proteins off the PEG-biotin layer.     

Mercuric triflate-catalyzed synthesis of 2-methylfurans from 1-alkyn-5-ones

[reaction: see text] 2-Methylfurans were prepared by an effective cyclization of 1-alkyn-5-ones in the presence of mercuric triflate as the catalyst under very mild reaction conditions with high catalytic turnover up to 100 times. Benzene, toluene, or dichloromethane was the solvent of choice.     

Immobilization of Lipase from Grey Mullet

Grey mullet (Mugil cephalus) lipase was isolated using para-aminobenzamidine agarose and immobilized on octyl Sepharose CL-4B (o-Sep). Immobilized grey mullet lipase (GMLi) had a 10?°C higher optimum temperature compared to the free enzyme and showed remarkable thermal stability. GMLi was most active within the pH range of 8.0?C9.5 with an optimum at 8.5. Immobilization also enhanced the storage stability and reusability of the enzyme with minimal changes in efficiency during repeated batches. GMLi showed variable stabilities in various organic solvents. A signal in the amide I absorption region of the FTIR spectrum of GMLi was attributed to the protein layer on o-Sep. The surface morphology of o-Sep was visualized on a Zeiss stereomicroscope as globular-shaped beads.     

Thermal activation of photoactivatable urocanase from Pseudomonas putida

The dark inactivation of urocanase from Pseudomonas putida is caused by the formation of a sulfite adduct of the tightly bound coenzyme, nicotinamide adenine dinucleotide. Photodissociation of this adduct by UV radiation restores the enzyme activity. Based on cold exhaustive dialysis the modification reaction appeared to be irreversible. However, we now report that sulfite modification of urocanase is reversible at higher temperatures. An Arrhenius plot of the thermal activation is linear (20-38 degrees C). The activation energy for the enzyme activation is 114 kJ mol-1. The substance that is photodissociated from inactive urocanase reacts with urocanase to reform the modified enzyme indicating that sulfite is not oxidized, or otherwise changed through these processes. Nucleophiles (sulfite, hydroxylamine, hydride, cyanide) are known to inhibit urocanase by forming adducts with nicotinamide adenine dinucleotide. Urocanase inactivated by hydride or cyanide is not reactivated thermally or photochemically. Urocanase inactivated by hydroxylamine and by glycylglycine can be reactivated by a thermal reaction. In conclusion, sulfite-modified urocanase, which is formed in cells, can be reactivated not only by sunlight but also at physiological temperatures.     

Naphthalene adsorption on activated carbons using solvents of different polarity

The hydrophobic-hydrophilic character of a series of microporous activated carbons was explored as a key factor in competitive adsorption of a non-polar compound from liquid phase. The selectivity of the carbon surface towards naphthalene was explored by performing the adsorption isotherms in water, cyclohexane and heptane. Solvent polarity and adsorbent hydrophobic character were found to strongly influence the adsorption capacity of naphthalene. In aqueous media, despite the non-polar character of the adsorbate, surface acidity lowered adsorption capacity. This is attributed to the competition of water from the adsorption sites, via H-bonding with surface functionalities and the formation of hydration clusters that reduce the accessibility and affinity of naphthalene to the inner pore structure. In organic media the uptake decreased due to competition of the hydrophobic solvent for the active sites of the carbon and to solvation effects. This competitive effect of the solvent is minimized in oxidized carbons as opposed to the trend obtained in aqueous solutions. The results confirmed that although adsorption of naphthalene strongly depends on the narrow microporosity of the adsorbent, competitive adsorption of the solvent for the active sites becomes important.     

Immobilization of invertase on porous membranes made from modified polysulfone

The activity of invertase that was immobilized within asymmetric ultrafiltration membranes was determined as a function of the immobilization mode such as adsorption, ionic interaction and covalent bonding. For these different bonding possibilities adequate membranes were prepared from chemically modified polysulfone fitted out with the corresponding substituents. The amount of enzyme was lowest for adsorption and highest for chemical fixation. In the latter case spacers were useful because substituents adjacent to the polymer backbone caused a relatively large loss of activity which can stem either from chemical reaction or from the hampered development of the appropriate conformational structure. Compared to the activity of the native invertase the fixation yielded a remarkable reduction of activity which was compensated for by the very extended stability of the bonded enzyme.     

Comparative evaluation of xerogel-based activated carbons synthesized from aliphatic aldehydes of different chain lengths

This work deals with examining the performance of xerogel-based activated carbons (XACs), which were synthesized from aliphatic aldehydes of different carbon chain lengths. These XACs were compared with those synthesized from commonly synthesized XACs. The performance of the new xerogels was determined by examining the thermo-gravimetric analysis (TGA) and Fourier transform infrared (FTIR); however, the XACs were studied using infrared spectra (IR), scanning electron microscopy (SEM), and their adsorption capacities in gas and aqueous media (nitrogen adsorption, iodine number, adsorption of phenol and methylene blue, MB). The adsorption behavior of these investigated XACs to MB was studied in detail, using the Langmuir and Freundlich adsorption equations, in addition to kinetic (Lagergren first-order and pseudo-second-order) and thermodynamic models. The results show that long -chain aldehydes have a significant effect on increasing the total pore volume (V_T). Glutaraldehyde-based carbon xerogel is recommended as an economically superior adsorbent with an S_BET x yield of 571.9 m²/g. XACs from glutaraldehyde and propionaldehyde have higher surface area than commonly synthesized ACs from formaldehyde (F), Phenol/F, Tanin/F-, Polybenzooxazine/F, and Pyrogallol/F. The best models used for MB adsorption onto XACs are Langmuir and pseudo-second-order kinetic equations. The negative values of thermodynamic parameter ΔGº and positive values of ΔHº indicate the MB adsorption process is spontaneous and endothermic.     

Preparation of nano-silver-supported activated carbon using different ligands

In this study, we investigated the effect of water soluble ligands [i.e., sodium borohydride (NaBH₄), polyvinyl alcohol, glucose and galactose] on the preparation of nano-silver-supported activated carbon (AC). Ligand-stabilized Ag nanoparticle dispersion characteristics were also compared with those of ligand-free Ag nanoparticles. The nanoparticle distribution was investigated using a scanning electron microscope (SEM) which enabled a qualitative analysis of ligand-dependent nanoparticle adsorption onto AC. Silver nanoparticles with average sizes ranging from 7 to 20 nm were synthesized with different coatings. In particular, silver nanoparticles reduced and stabilized by NaBH₄ were found to have a dense and homogenous dispersion of sizes in the range of 100–400 nm on the AC surface. These particles also seemed to remain on the AC surface after rinsing with water. The distribution of silver nanoparticles prepared in the presence of NaBH₄/PVA was not as good as the one prepared with NaBH₄. Their aggregate size varied from 300 to 600 nm on the AC surface and particles greater than 500 nm were eliminated from the AC surface upon rinsing with water. Glucose- and galactose-stabilized silver nanoparticles did not display an extensive adsorption and their adsorption seemed to be poor. However, glucose-stabilized silver nanoparticles could still be detectable to some extent after rinsing, while galactose-stabilized ones could not. Antimicrobial studies showed that all silver-containing carbons studied in this study inhibit bacterial growth and act as bacteriostatic agents.     

NMR spectroscopy as a tool to investigate the degradation of aromatic compounds by a Pseudomonas putida strain

Pseudomonas putida strain KT2442, harbouring the pWW0 TOL plasmid, was grown with a number of different homologous aromatic acids as carbon sources. Small samples of liquid culture supernatant were collected and directly analysed by 2D NMR spectroscopy. In all cases similar compounds with olefinic signals were observed to accumulate. To elucidate the structures of these compounds, 2D NMR experiments with 500 and 600 MHz spectrometers equipped with a CryoProbe (Bruker BioSpin) were performed on samples obtained from a culture growing on 4‐methylbenzoate and, for ¹³C spectroscopy, on ¹³C‐labelled 4‐methylbenzoate. In all cases a 1,2‐dihydroxycyclohexa‐3,5‐diene‐carboxylate derivative was identified. The use of this technique helped us to identify easily some metabolites that were released into the solution by bacteria and to follow their secretion as a function of time. The high sensitivity of the present approach allowed a clear and rapid acquisition of spectra, notwithstanding the low concentration of the compounds. The benefits of introducing the use of NMR cryoprobes to perform metabolic pathway studies is demonstrated. Copyright © 2003 John Wiley & Sons, Ltd.     

Immobilization and Stabilization of Beta-Xylosidases from Penicillium janczewskii

β-Xylosidases are critical for complete degradation of xylan, the second main constituent of plant cell walls. A minor β-xylosidase (BXYL II) from Penicillium janczewskii was purified by ammonium sulfate precipitation (30% saturation) followed by DEAE-Sephadex chromatography in pH 6.5 and elution with KCl. The enzyme presented molecular weight (MW) of 301 kDa estimated by size exclusion chromatography. Optimal activity was observed in pH 3.0 and 70–75 °C, with higher stability in pH 3.0–4.5 and half-lives of 11, 5, and 2 min at 65, 70, and 75 °C, respectively. Inhibition was moderate with Pb⁺² and citrate and total with Cu⁺², Hg⁺², and Co⁺². Partially purified BXYL II and BXYL I (the main β-xylosidase from this fungus) were individually immobilized and stabilized in glyoxyl agarose gels. At 65 °C, immobilized BXYL I and BXYL II presented half-lives of 4.9 and 23.1 h, respectively, therefore being 12.3-fold and 33-fold more stable than their unipuntual CNBr derivatives (reference mimicking soluble enzyme behaviors). During long-term incubation in pH 5.0 at 50 °C, BXYL I and BXYL II glyoxyl derivatives preserved 85 and 35% activity after 25 and 7 days, respectively. Immobilized BXYL I retained 70% activity after 10 reuse cycles of p-nitrophenyl-β-D-xylopyranoside hydrolysis.

     

木瓜蛋白酶的固定化研究

木瓜蛋白酶具有广谱的蛋白水解酶活性,广泛地应用于啤酒、饮料的澄清,肉类嫩化和复配消化药物等方面。近年来,为了扩大该酶在啤洒澄清上的应用,一些研究者致力于探索该酶的固定化研究,以提高该酶的利用效率,降低生产成本。     

Gerbils of a seizure-sensitive strain have a mitochondrial inner membrane protein with different isoelectric points from those of a seizure-resistant strain

The distribution of proteins in the cerebral cortex of a seizure-sensitive (SS) strain of gerbil and its seizure-resistant (SR) counterpart was profiled using two-dimensional gel electrophoresis. A series of proteins of similar molecular weight (around 83 kDa) showed small but consistent differences in their isoelectric point (pI) with indistinguishable profiles of distribution between the two strains. Amino acid sequences of peptides produced by limited proteolysis of each protein in the spots from the strains were identical or highly homologous to those of mitofilin, a mitochondrial inner membrane protein (IMMT) in humans. Analysis of cDNA sequences revealed the proteins of these spots to be gerbil mitofilin-like proteins (gIMMT), with a few base substitutions between SS and SR strains, in particular within a region near a putative transmembrane domain that is highly conserved in humans and gerbils. The amino acid at the site was acidic, Glu in humans and Asp in the strain SR of gerbil and a neutral, Asn in strain SS. In addition to these base substitutions, production of multiple species of mRNA for gIMMT by alternative splicing was observed.     

Stress–strain relations of crosslinked rubbers under different types of strain

Experimental data for the stresses and the deformations for crosslinked rubbers at uniaxial and symmetrical and asymmetrical biaxial extension and pure shear are given. Stressed states up to 100% extension are described by a single parameter, the highly elastic potential of Bartenev and Khazanovich. The classical statistical potential of Kuhn-James-Guth-Treloar is not in agreement with experimental data, as shear modulus G has different values for different types of stressed states.